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Formation network covalent solids

The formation of covalent cross-linking in liquid-crystalline polymers is useful to lock in the molecular order in solid states, which leads to static functionality [114, 115]. For hydrogen-bonded mesogenic networks, the use of the dynamic nature of H-bonding induces dynamic properties [108, 109]. It is important to choose an appropriate method of cross-linking for the purpose of the use of network materials. [Pg.123]

In protein microarrays, capture molecules need to be immobilized in a functional state on a solid support. In principle, the format of the assay system does not limit the choice of appropriate surface chemistry. The same immobilization procedure can be applied for both planar and bead-based systems. Proteins can be immobilized on various surfaces (Fig. 1) (12). Two-dimensional polystyrene, polylysine, aminosilane, or aldehyde, epoxy- or thiol group-coated surfaces can be used to immobilize proteins via noncovalent or covalent attachment (13,14). Three-dimensional supports like nitrocellulose or hydrogel-coated surfaces enable the immobilization of the proteins in a network structure. Larger quantities of proteins can be immobilized and kept in a functional state. Affinity binding reagents such as protein A, G, and L can be used to immobilize antibodies (15), streptavidin is used for biotinylated proteins (16), chelate for His-tagged proteins (17, 18), anti-GST antibodies for GST fusion proteins (19), and oligonucleotides for cDNA or mRNA-protein hybrids (20). [Pg.201]


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See also in sourсe #XX -- [ Pg.281 , Pg.281 ]

See also in sourсe #XX -- [ Pg.281 , Pg.281 ]




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Covalent network

Covalent solids

Network covalent solid

Network formation

Network solids

Solid formation

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